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US20030134431A1 - High throughput screening assay systems in microscale fluidic devices - Google Patents

High throughput screening assay systems in microscale fluidic devices
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US20030134431A1
US20030134431A1US10/279,496US27949602AUS2003134431A1US 20030134431 A1US20030134431 A1US 20030134431A1US 27949602 AUS27949602 AUS 27949602AUS 2003134431 A1US2003134431 A1US 2003134431A1
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channels
channel
component
biochemical system
substrate
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J. Parce
Anne Kopf-Sill
Luc Bousse
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Caliper Life Sciences Inc
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Caliper Technologies Corp
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Abstract

The present invention provides novel microfluidic devices and methods that are useful for performing high-throughput screening assays. In particular, the devices and methods of the invention are useful in screening large numbers of different compounds for their effects on a variety of chemical, and preferably, biochemical systems.

Description

Claims (97)

What is claimed is:
1. An apparatus for screening test compounds for an effect on a biochemical system, comprising:
a substrate having at least one surface;
at least two intersecting channels fabricated into said surface of said substrate, at least one of said at least two intersecting channels having at least one cross-sectional dimension in the range from about 0.1 to about 500 μm;
a source of a plurality of different test compounds fluidly connected to a first of said at least two intersecting channels;
a source of at least one component of said biochemical system fluidly connected to a second of said at least two intersecting channels;
a fluid direction system for flowing said at least one component within said second of said at least two intersecting channels and for introducing said different test compounds from said first to said second of said at least two intersecting channels;
a cover mated with said surface; and
a detection zone in said second channel for detecting an effect of said test compound on said biochemical system.
2. The apparatus ofclaim 1, wherein said fluid direction system generates a continuous flow of said at least first component along said second of said at least two intersecting channels, and periodically injects a test compound from said first channel into said second channel.
3. The apparatus ofclaim 1, further comprising a source of a second component of said biochemical system, and a third channel fabricated into said surface, said third channel fluidly connecting at least one of said at least two intersecting channels with said source of said second component of said biochemical system.
4. The apparatus ofclaim 3, wherein said fluid direction system generates a continuous flow of a mixture of said first component and said second component along said second of said at least two intersecting channels, and periodically injects a test compound from said first channel into said second channel.
5. The apparatus ofclaim 1, wherein said fluid direction system continuously flows said plurality of different test compounds from said first into said second of said at least two intersecting channels, each of said plurality of different test compounds being separated by a fluid spacer.
6. The apparatus ofclaim 1, wherein said fluid direction system comprises:
at least three electrodes, each electrode being in electrical contact with said at least two intersecting channels on a different side of an intersection formed by said at least two intersecting channels; and
a control system for concomitantly applying a variable voltage at each of said electrodes, whereby movement of said test compounds or said at least first component in said at least two intersecting channels are controlled.
7. The apparatus ofclaim 1, wherein said detection system includes a detection window in said second channel.
8. The apparatus ofclaim 7, wherein said detection system is a fluorescent detection system.
9. The apparatus ofclaim 1, wherein said substrate is planar.
10. The apparatus ofclaim 1, wherein said substrate comprises etched glass.
11. The apparatus ofclaim 1, wherein said substrate comprises etched silicon.
12. The apparatus ofclaim 1, further comprising an insulating layer disposed over said etched silicon substrate.
13. The apparatus ofclaim 1, wherein said substrate is a molded polymer.
14. The apparatus ofclaim 1, wherein said at least one component of a biochemical system comprises an enzyme, and a substrate which produces a detectable signal when reacted with said enzyme.
15. The apparatus ofclaim 14, wherein said substrate is selected from the group consisting of chromogenic and fluorogenic substrates.
16. The apparatus ofclaim 1, wherein said at least first component of a biochemical system comprises a receptor/ligand binding pair, wherein at least one of said receptor or ligand has a detectable signal associated therewith.
17. The apparatus ofclaim 1, wherein said first component of a biochemical system comprises a receptor/ligand binding pair, wherein binding of said receptor to said ligand produces a detectable signal.
18. The apparatus ofclaim 1, the apparatus further comprising a plurality of electrodes in a plurality of reservoirs fluidly connected to one or more of said intersecting channels and a control system for concomitantly applying a voltage to each of said electrodes, whereby movement of said first component in said at least two intersecting channels is controlled.
19. The apparatus ofclaim 18, wherein the apparatus minimizes degradation of chemical species present in said reservoirs or said intersecting channels.
20. The apparatus ofclaim 19, wherein the apparatus further comprises one or more component for reducing electroosmotic flow, selected from the group consisting of:
a frit on one or more of the electrodes, which frit reduces electroosmotic flow towards the one or more electrodes;
a large channel between at least two of said reservoirs, which large channel limits diffusion of said chemical species, the channel having low electroosmotic flow;
a narrow channel between at least two of said reservoirs, which narrow channel limits diffusion of said chemical species, the narrow channel treated to reduce electroosmotic flow;
a filled channel between at least two of said reservoirs, which filled channel comprises a matrix to limit transport of said chemical species through the filled channel, the filled channel thereby having low electroosmotic flow;
a high reservoir having a fluid level higher than at least one low reservoir, which high reservoir is fluidly connected to said low reservoir, which low reservoir comprises an electrode, wherein fluid pressure between the high reservoir and the low reservoir reduces electroosmotic flow towards the electrode; and,
a dual reservoir system with a first reservoir fluidly connected through a connecting channel to a narrow diameter second reservoir adapted to receive one of the plurality of electrodes, said narrow diameter second reservoir adapted to draw fluid by capillary electrophoresis towards the one electrode, thereby countering electroosmotic flow in the connecting channel.
21. An apparatus for detecting an effect of a test compound on a biochemical system, comprising:
a substrate having at least one surface;
a plurality of reaction channels fabricated into said surface;
at least two transverse channels fabricated into said surface, each of said plurality of reaction channels being fluidly connected to a first of said at least two transverse channels at a first point in said reaction channels, and fluidly connected to a second of said at least two transverse channels at a second point in said reaction channels, said at least two transverse channels and said plurality of reaction channels each having at least one cross-sectional dimension in the range from about 0.1 to about 500 μm;
a source of at least one component of said biochemical system, said source of at least one component of said biochemical system being fluidly connected to each of said plurality of reaction channels;
a source of test compounds fluidly connected to said first of said at least two transverse channels;
a fluid direction system for controlling movement of said test compound and said at least one component within said at least two transverse channels and said plurality of reaction channels;
a cover mated with said surface; and
a detection system for detecting an effect of said test compound on said biochemical system.
22. The apparatus ofclaim 21, wherein said fluid control system comprises:
a plurality of individual electrodes, each in electrical contact with each terminus of said at least two transverse channels; and
a control system for concomitantly applying a variable voltage at each of said electrodes, whereby movement of said test compounds or said at least first component in said at least two transverse channels and said plurality of reaction channels are controlled.
23. The apparatus ofclaim 21, wherein each of said plurality of reaction channels comprises a bead resting well at said first point in said plurality of reaction channels.
24. The apparatus ofclaim 21, wherein said source of at least one component of a biochemical system is fluidly connected to said plurality of reaction channels by a third transverse channel, said third transverse channel having at least one cross sectional dimension in a range of from 0.1 to 500 μm and being fluidly connected to each of said plurality of reaction channels at a third point in said reaction channels.
25. The apparatus ofclaim 21, wherein said third point in said reaction channels is intermediate to said first and second points in said reaction channels.
26. The apparatus ofclaim 25, further comprising a particle retention zone in each of said plurality of reaction channels, between said third and said second points in said plurality of reaction channels.
27. The apparatus ofclaim 26, wherein said particle retention zone comprises a particle retention matrix.
28. The apparatus ofclaim 26, wherein said particle retention zone comprises a microstructural filter.
29. The apparatus ofclaim 21, wherein said plurality of reaction channels comprises a plurality of parallel reaction channels fabricated into said surface of said substrate and said at least two transverse channels are connected at opposite ends of each of said parallel reaction channels.
30. The apparatus ofclaim 21, wherein said at least two transverse channels are fabricated on said surface of said substrate in inner and outer concentric channels, respectively, and said plurality of reaction channels extend radially from said inner concentric channel to said outer concentric channel.
31. The apparatus ofclaim 30, wherein said detection system comprises a detection window in said second channel.
32. The apparatus ofclaim 30, wherein said detection system is a fluorescent detection system.
33. The apparatus ofclaim 21, wherein said substrate is planar.
34. The apparatus ofclaim 21, wherein said substrate comprises etched glass.
35. The apparatus ofclaim 21, wherein said substrate comprises etched silicon.
36. The apparatus ofclaim 21, further comprising an insulating layer disposed over said etched silicon substrate.
37. The apparatus ofclaim 21, wherein said substrate is a molded polymer.
38. The apparatus ofclaim 21, wherein said at least one component of a biochemical system comprises an enzyme, and an enzyme substrate which produces a detectable signal when reacted with said enzyme.
39. The apparatus ofclaim 38, wherein said enzyme substrate is selected from the group consisting of chromogenic and fluorogenic substrates.
40. The apparatus ofclaim 21, wherein said at least first component of a biochemical system comprises a receptor/ligand binding pair, wherein at least one of said receptor or ligand has a detectable signal associated therewith.
41. The apparatus ofclaim 21, wherein said first component of a biochemical system comprises a receptor/ligand binding pair, wherein binding of said receptor to said ligand produces a detectable signal.
42. A method of determining whether a sample contains a compound capable of affecting a biochemical system, comprising:
providing a substrate having at least a first surface, and at least two intersecting channels fabricated in said first surface, at least one of said at least two intersecting channels having at least one cross-sectional dimension in a range from 0.1 to 500 μm;
flowing a first component of a biochemical system in a first of said at least two intersecting channels;
flowing said sample from a second channel into said first channel whereby said sample contacts said first component of said biochemical system; and
detecting an effect of said at least sample on said biochemical system.
43. The method ofclaim 42, wherein said at least first component of a biochemical system comprises at least one member of an antibody/antigen binding pair, wherein said antibody is specifically immunoreactive with said antigen.
44. The method ofclaim 42, wherein said at least first component of a biochemical system comprises an antibody and an antigen specifically reactive with said antibody.
45. The method ofclaim 42, wherein one of said antibody or antigen comprises a detectable labelling group.
46. The method ofclaim 42, wherein said at least first component of a biochemical system comprises at least one member of a receptor/ligand binding pair.
47. The method ofclaim 42, wherein said at least first component of a biochemical system comprises a receptor and a ligand capable of specifically binding to said ligand.
48. The method ofclaim 42, wherein said sample is derived from a patient.
49. The method ofclaim 48, wherein said sample is blood-derived.
50. The method ofclaim 42, wherein said detecting step comprises measuring a parameter of said biochemical system in the presence and absence of said sample, and comparing the measured parameter in the presence of said sample to the measured parameter in the absence of said sample, a change in said parameter being indicative that said sample has an effect on said biochemical system.
51. An apparatus for screening test compounds for an effect on a biochemical system, comprising:
a substrate having at least one surface, and comprising at least two intersecting channels fabricated into said surface of said substrate, at least one of said at least two intersecting channels having at least one cross-sectional dimension in the range from about 0.1 to about 500 μm;
a source of a sample fluidly connected to a first of said at least two intersecting channels;
a source of at least one component of said biochemical system fluidly connected to a second of said at least two intersecting channels;
a fluid direction system for flowing said at least one component within said second of said at least two intersecting channels and for introducing said sample from said first to said second of said at least two intersecting channels;
a cover mated with said surface; and
a detection zone in said second channel for detecting an effect of said sample on said biochemical system.
52. A method of screening a plurality of test compounds for an effect on a biochemical system, comprising:
providing a substrate having at least a first surface, and at least two intersecting channels fabricated in said first surface, at least one of said at least two intersecting channels having at least one cross-sectional dimension in a range from 0.1 to 500 μm;
flowing a first component of a biochemical system in a first of said at least two intersecting channels;
flowing at least a first test compound from a second channel into said first channel whereby said first test compound contacts said first component of said biochemical system; and
detecting an effect of said at least first test compound on said biochemical system.
53. The method ofclaim 52, wherein said at least first component of a biochemical system produces a detectable signal representative of a function of said biochemical system.
54. The method ofclaim 52, wherein said at least first component further comprises an indicator compound which interacts with said first component to produce a detectable signal representative of a functioning of said biochemical system.
55. The method ofclaim 52, wherein said first component of a biochemical system comprises an enzyme and a substrate for said enzyme, wherein action of said enzyme on said substrate produces a detectable signal.
56. The method ofclaim 52, wherein said first component of a biochemical system comprises a receptor/ligand binding pair, wherein at least one of said receptor or ligand has a detectable signal associated therewith.
57. The method ofclaim 52, wherein said first component of a biochemical system comprises a receptor/ligand binding pair, wherein binding of said receptor to said ligand produces a detectable signal.
58. The method ofclaim 52, wherein said at least first component of a biochemical system is a biological barrier and said effect of said at least first test compound is an ability of said test compound to traverse said barrier.
59. The method ofclaim 58, wherein said barrier is selected from the group consisting of an epithelial or an endothelial layer.
60. The method ofclaim 52, wherein said at least first component of a biochemical system comprises cells, and said detecting step comprises determining an effect of said test compound on said cells.
61. The method ofclaim 60, wherein said cells are capable of producing a detectable signal corresponding to a cellular function, and said detecting step comprises detecting an effect of said test compound on said cellular function by detecting a level of said detectable signal.
62. The method ofclaim 60, wherein said detecting step comprises detecting an effect of said test compound on viability of said cells.
63. A method of screening a plurality of test compounds for an effect on a biochemical system, comprising:
providing a substrate having at least a first surface, and at least two intersecting channels fabricated in said first surface, at least one of said at least two intersecting channels having at least one cross-sectional dimension in a range from 0.1 to 500 μm;
continuously flowing a first component of a biochemical system in a first channel of said at least two intersecting channels;
periodically introducing a different test compound into said first channel from a second channel of said at least two intersecting channels; and
detecting an effect of said test compound on said at least first component of a biochemical system.
64. The method ofclaim 63, wherein said step of periodically introducing comprises flowing a plurality of different test compounds into said first channel from a second channel of said at least two intersecting channels, each of said plurality of different test compounds being physically isolated from each other of said plurality of different test compounds.
65. The method ofclaim 63, wherein said at least first component of a biochemical system produces a detectable signal representative of a function of said biochemical system.
66. The method ofclaim 65, wherein said detecting comprises monitoring said detectable signal from said continuously flowing first component at a point on said first channel, said detectable signal having a steady state intensity, and wherein said effect of said interaction between said first component and said test compound comprises a deviation from said steady state intensity of said detectable signal.
67. The method ofclaim 65, wherein said at least first component further comprises an indicator compound which interacts with said first component to produce a detectable signal representative of a functioning of said biochemical system.
68. The method ofclaim 67, wherein said first component of a biochemical system comprises an enzyme and said indicator compound comprises a substrate for said enzyme, wherein action of said enzyme on said substrate produces a detectable signal.
69. The method ofclaim 65, wherein said at least first component of a biochemical system comprises a receptor/ligand binding pair, wherein at least one of said receptor or ligand has a detectable signal associated therewith.
70. The method ofclaim 69, wherein said receptor and said ligand flow along said first channel at different rates.
71. The method ofclaim 65, wherein said first component of a biochemical system comprises a receptor/ligand binding pair, wherein binding of said receptor to said ligand produces a detectable signal.
72. The method ofclaim 63, wherein said at least first component of a biochemical system comprises cells, and said detecting step comprises determining an effect of said test compound on said cells.
73. The method ofclaim 72, wherein said cells are capable of producing a detectable signal corresponding to a cellular function, and said detecting step comprises detecting an effect of said test compound on said cellular function by detecting a level of said detectable signal.
74. The method ofclaim 72, wherein said detecting step comprises detecting an effect of said test compound on viability of said cells.
75. A method of screening a plurality of different test compounds for an effect on a biochemical system, comprising:
providing a substrate having at least a first surface, and a plurality of reaction channels fabricated in said first surface, each of said plurality of reaction channels being fluidly connected to at least two transverse channels fabricated in said surface;
introducing at least a first component of a biochemical system into said plurality of reaction channels;
flowing a plurality of different test compounds through at least one of said at least two transverse channels, each of said plurality of test compounds being introduced into said at least one transverse channels in a separate subject material region;
directing each of said plurality of different test compounds into a separate one of said plurality of reaction channels; and
detecting an effect of each of said test compounds on said at least one component of said biochemical system.
76. The method ofclaim 75, wherein said at least first component of said biochemical system produces a flowable detectable signal representative of a function of said biochemical system.
77. The method ofclaim 76, wherein said detectable flowable signal produced in each of said plurality of reaction channels is flowed into and through said second transverse channel, each of said detectable flowable signals produced in each of said plurality of reaction channels being physically isolated from each other of said detectable flowable signals, whereupon each of said detectable flowable signals is separately detected.
78. The method ofclaim 76, wherein said flowable signal comprises a soluble signal.
79. The method ofclaim 78, wherein said soluble signal is selected from fluorescent or colorimetric signals.
80. The method ofclaim 75, wherein said at least first component further comprises an indicator compound which interacts with said first component to produce a detectable signal representative of a functioning of said biochemical system.
81. The method ofclaim 80, wherein said first component of a biochemical system comprises an enzyme and said indicator compound comprises a substrate for said enzyme, wherein action of said enzyme on said substrate produces a detectable signal.
82. The method ofclaim 75, wherein said at least first component of a biochemical system comprises a receptor/ligand binding pair, wherein at least one of said receptor or ligand has a detectable signal associated therewith.
83. The method ofclaim 75, wherein said first component of a biochemical system comprises a receptor/ligand binding pair, wherein binding of said receptor to said ligand produces a detectable signal.
84. The method ofclaim 75, wherein said at least first component of a biochemical system comprises cells, and said detecting step comprises determining an effect of said test compound on said cells.
85. The method ofclaim 84, wherein said cells are capable of producing a detectable signal corresponding to a cellular function, and said detecting step comprises detecting an effect of said test compound on said cellular function by detecting a level of said detectable signal.
86. The method ofclaim 85, wherein said detecting step comprises detecting an effect of said test compound on viability of said cells.
87. The method ofclaim 75, wherein each of said plurality of different test compounds is immobilized upon a separate bead, and said step of directing each of said plurality of different test compounds into a separate one of said plurality of reaction channels comprises:
lodging one of said separate beads at an intersection of said first transverse channel and each of said plurality of reaction channels; and
controllably releasing said test compounds from each of said separate beads into each of said plurality of reaction channels.
88. The use of a microfluidic system containing at least a first substrate having a first channel and a second channel intersecting said first channel, at least one of said channels having at least one cross-sectional dimension in a range from 0.1 to 500 μm, in order to test the effect of each of a plurality of test compounds on a biochemical system.
89. A use ofclaim 88, wherein said biochemical system flows through one of said channels substantially continuously, enabling sequential testing of said plurality of test compounds.
90. A use ofclaim 88, orclaim 89, wherein the provision of a plurality of reaction channels in said first substrate enables parallel exposure of a plurality of test compounds to at least one biochemical system.
91. A use of any of claims88,89, or90 wherein each test compound is physically isolated from adjacent test compounds.
92. The use of a substrate carrying intersecting channels in screening test materials for effect on a biochemical system by flowing said test materials and biochemical system together using said channels.
93. A use ofclaim 92, wherein at least one of said channels has at least one cross-sectional dimension of range 0.1 to 500 μm.
94. An assay utilizing a use of any one ofclaims 88 to93.
95. An apparatus for detecting an effect of a test compound on a biochemical system, comprising a substrate having at least one surface with a plurality of reaction channels fabricated into the surface.
96. An apparatus as claimed inclaim 95, having at least two transverse channels fabricated into the surface, wherein each of the plurality of reaction channels is fluidly connected to a first of the at least two transverse channels at a first point in each of the reaction channels, and fluidly connected to a second transverse channel at a second point in each of the reaction channels.
97. Assay apparatus including an apparatus as claimed inclaim 95 orclaim 1.
US10/279,4961996-06-282002-10-24High throughput screening assay systems in microscale fluidic devicesExpired - LifetimeUS7091048B2 (en)

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US10/279,496US7091048B2 (en)1996-06-282002-10-24High throughput screening assay systems in microscale fluidic devices
US10/821,503US7067263B2 (en)1996-06-282004-04-08High throughput screening assay systems in microscale fluidic devices

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US08/671,987US5942443A (en)1996-06-281996-06-28High throughput screening assay systems in microscale fluidic devices
US08/761,575US6046056A (en)1996-06-281996-12-06High throughput screening assay systems in microscale fluidic devices
US08/881,696US6267858B1 (en)1996-06-281997-06-24High throughput screening assay systems in microscale fluidic devices
US09/132,963US6479299B1 (en)1996-06-281998-08-12Pre-disposed assay components in microfluidic devices and methods
US10/279,496US7091048B2 (en)1996-06-282002-10-24High throughput screening assay systems in microscale fluidic devices

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US09/214,035Expired - LifetimeUS6429025B1 (en)1996-06-281997-06-24High-throughput screening assay systems in microscale fluidic devices
US09/044,557Expired - LifetimeUS6274337B1 (en)1996-06-281998-03-19High throughput screening assay systems in microscale fluidic devices
US09/044,587Expired - LifetimeUS6413782B1 (en)1996-06-281998-03-19Methods of manufacturing high-throughput screening systems
US09/132,963Expired - LifetimeUS6479299B1 (en)1996-06-281998-08-12Pre-disposed assay components in microfluidic devices and methods
US09/196,535Expired - LifetimeUS6306659B1 (en)1996-06-281998-11-20High throughput screening assay systems in microscale fluidic devices
US09/612,587Expired - LifetimeUS6399389B1 (en)1996-06-282000-07-07High throughput screening assay systems in microscale fluidic devices
US09/718,236Expired - LifetimeUS6630353B1 (en)1996-06-282000-11-21High throughput screening assay systems in microscale fluidic devices
US09/718,235Expired - LifetimeUS6558960B1 (en)1996-06-282000-11-21High throughput screening assay systems in microscale fluidic devices
US10/279,496Expired - LifetimeUS7091048B2 (en)1996-06-282002-10-24High throughput screening assay systems in microscale fluidic devices
US10/637,730AbandonedUS20040028567A1 (en)1996-06-282003-08-07High throughput screening assay systems in microscale fluidic devices
US10/821,503Expired - Fee RelatedUS7067263B2 (en)1996-06-282004-04-08High throughput screening assay systems in microscale fluidic devices
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US09/044,557Expired - LifetimeUS6274337B1 (en)1996-06-281998-03-19High throughput screening assay systems in microscale fluidic devices
US09/044,587Expired - LifetimeUS6413782B1 (en)1996-06-281998-03-19Methods of manufacturing high-throughput screening systems
US09/132,963Expired - LifetimeUS6479299B1 (en)1996-06-281998-08-12Pre-disposed assay components in microfluidic devices and methods
US09/196,535Expired - LifetimeUS6306659B1 (en)1996-06-281998-11-20High throughput screening assay systems in microscale fluidic devices
US09/612,587Expired - LifetimeUS6399389B1 (en)1996-06-282000-07-07High throughput screening assay systems in microscale fluidic devices
US09/718,236Expired - LifetimeUS6630353B1 (en)1996-06-282000-11-21High throughput screening assay systems in microscale fluidic devices
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US11/176,805AbandonedUS20050241941A1 (en)1996-06-282005-07-06High throughput screening assay systems in microscale fluidic devices

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US6274337B1 (en)2001-08-14

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